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粪链球菌对2-酮葡萄糖酸盐的发酵作用

2-KETOGLUCONATE FERMENTATION BY STREPTOCOCCUS FAECALIS.

作者信息

GODDARD J L, SOKATCH J R

出版信息

J Bacteriol. 1964 Apr;87(4):844-51. doi: 10.1128/jb.87.4.844-851.1964.

Abstract

Goddard, J. L. (University of Oklahoma School of Medicine, Oklahoma City), and J. R. Sokatch. 2-Ketogluconate fermentation by Streptococcus faecalis. J. Bacteriol. 87:844-851. 1964.-Streptococcus faecalis 10Cl did not grow with 2-ketogluconate alone as an energy source, but did grow when gluconate was added. More growth was obtained than could be accounted for by the gluconate alone. The requirement for gluconate in the stimulation of growth on 2-ketogluconate was found to be stoichiometric, not catalytic. Glucose did not replace gluconate in this phenomenon, apparently owing to the repression of the 2-ketogluconate pathway by glucose. Resting cells grown on a combination of gluconate and 2-ketogluconate did ferment 2-ketogluconate without added gluconate. Fermentation balance studies with resting cells detected the following products in moles (per mole of 2-ketogluconate): carbon dioxide, 0.98; lactic acid, 0.19; formic acid, 1.42; acetic acid, 0.70; and ethanol, 0.42. 2-Ketogluconate-1-C(14) and -2-C(14) were prepared and fermented. The data were interpreted to show that 90% of the substrate was decarboxylated to carbon dioxide and pentose phosphate. Pentose phosphate was then fermented to pyruvate through the sedoheptulose diphosphate variation of the pentose phosphate pathway found in this organism. The other 10% of the substrate was converted to pyruvate by way of the Entner-Doudoroff pathway. Calculations of the energy available by the above combination of pathways indicated that about 2.3 moles of adenosine triphosphate per mole of 2-ketogluconate could be obtained if the energy available in acetate formation is conserved through the acetokinase reaction.

摘要

戈达德,J. L.(俄克拉荷马大学医学院,俄克拉荷马城),以及J. R. 索卡奇。粪肠球菌对2-酮葡糖酸盐的发酵。《细菌学杂志》87:844 - 851。1964年。——粪肠球菌10Cl单独以2-酮葡糖酸盐作为能量来源时不能生长,但添加葡糖酸盐后能够生长。获得的生长量比仅由葡糖酸盐所能解释的要多。发现在2-酮葡糖酸盐上刺激生长时对葡糖酸盐的需求是化学计量的,而非催化的。葡萄糖在这种现象中不能替代葡糖酸盐,显然是由于葡萄糖对2-酮葡糖酸盐途径的阻遏作用。在葡糖酸盐和2-酮葡糖酸盐的组合培养基上生长的静息细胞在不添加葡糖酸盐的情况下确实能发酵2-酮葡糖酸盐。对静息细胞进行的发酵平衡研究检测到以下产物(每摩尔2-酮葡糖酸盐的摩尔数):二氧化碳,0.98;乳酸,0.19;甲酸,1.42;乙酸,0.70;以及乙醇,0.42。制备并发酵了2-酮葡糖酸盐-1-C(14)和-2-C(14)。数据解释表明90%的底物脱羧生成二氧化碳和戊糖磷酸。然后戊糖磷酸通过该生物体中发现的戊糖磷酸途径的景天庚酮糖二磷酸变体发酵生成丙酮酸。另外10%的底物通过恩特纳-杜德洛夫途径转化为丙酮酸。通过上述途径组合计算可得的能量表明,如果通过乙酰激酶反应保存乙酸形成过程中可用的能量,每摩尔2-酮葡糖酸盐大约可获得2.3摩尔三磷酸腺苷。

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